CN101954095B - Targeted gene delivery to non-phagocytic mammalian cells via bacterially derived intact minicells - Google Patents
Targeted gene delivery to non-phagocytic mammalian cells via bacterially derived intact minicells Download PDFInfo
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Abstract
A method of targeting bacterially-derived, intact minicells to specific, non-phagocytic mammalian cells employs bispecific ligands to deliver nucleic acids efficiently to the mammalian cells. Bispecific ligands, comprising (i) a first arm that carries specificity for a bacterially-derived minicell surface structure and (ii) a second arm that carries specificity for a non-phagocytic mammalian cell surface receptor are useful for targeting minicells to specific, non-phagocytic mammalian cells and causing endocytosis of minicells by non-phagocytic cells.
Description
The application is that the China national application number of December in 2004 application on the 8th is 200480041370.4, international application no is (PCT/IB2004/004406), and denomination of invention is divided an application for the patent application of " target gene being delivered to non-phagocytic mammalian cells by the complete minicell that is derived from antibacterial ".
The cross reference of related application
The application requires the benefit of priority of the United States Patent (USP) provisional application case 60/527,764 of December in 2003 submission on the 9th, during the whole content of this provisional application case is incorporated herein thus.
Background of invention
The present invention relates to the non-method and composition of engulfing host cell of antibacterial minicell carrier targeting, especially (but being not special) is in the gene therapy scope.The present invention uses the not only specific binding two special moleculars to minicell surface texture but also specific binding to host cell surface structure (for example receptor).By the reciprocal action between mediation minicell carrier and the non-phagosome host cell, the bispecific part can be with oligonucleotide and polynucleotide targeted delivery to host cell.
The target of gene therapy is that one or more exogenous genes are inserted in the body cell to close a gene, replace a damaged gene or to express a gene outcome that prevention or therapeutical effect can be provided.The progress of recently gene therapy focuses on and various exogenous gene is introduced into method in the receptor mammalian genes group.Referring to people such as Romano, 1998,1999; Balicki and Beutler, 2002; The people such as Wadhwa, 2002; Reach the people such as Thomas, 2003.These progress relate to uses viral vector (the existing mankind have again non-human) and non-virus carrier (for example DNA-liposome complex).
Although each carrier system has its advantage, every kind has the remarkable shortcoming that limits some clinical practices equally.Particularly, viral vector causes serious safety problem, it comprises with wild-type virus recombinates, the possibility of embedding and tumorigenesis, animal virus vector is to the intrinsic toxicity of mammalian cell, the immunosuppressant of virus induction, the answer of attenuated virus virulence, and such as the adverse effects such as inflammatory reaction that caused by existing immunity.There is practical problems equally in viral vector, and for example recombinant virus manufacturing and the difficulty that distributes are low stable, and the carrier finite capacity can not carry a large amount of foreign DNAs.Non-virus carrier has the lower shortcoming of the common efficient of gene delivery.
For being devoted to solve these shortcomings, PCT/IB02/04632 has set forth the complete minicell of restructuring that contains therapeutic nucleic acid molecule.This class minicell be external and body in oligonucleotide and the delivery of polynucleotides effective carrier to host cell.For example, the PCT/IB02/04632 proof can be delivered to the restructuring minicell that carries the mammalian gene expression plasmid phagocyte (for example macrophage) and non-phagocytic cell (but the example of successful candidate in the imperial examinations at the provincial level in the Ming and Qing dynasties's class breast cancer cell illustrates).This application case shows that equally the intraperitoneal minicell of recombinating causes recombiant plasmid to be delivered to the immune system phagocyte, and can cause the serum antibody response to coded protein.
Although by minicell with gene delivery to cytophagous efficient very high (40-60%), so far with the efficient of gene delivery to non-phagocytic cell always quite low (3% to 5%).Estimate that this will seriously limit clinical practice, because a lot of potential indication of gene therapy relates to endothelium and other non-phagocytic cell.For example most of cancer is not the phagocyte cancer, and it is believed that shortage cell or organ specific carrier can not be used for effectively this class cancer for the treatment of.
Similarly specificity lacks the application that has equally hindered the non-small cell carrier, and the whole bag of tricks in the exploitation is devoted to address this problem.Referring to Wickham, 2003.A kind of method utilization is present in receptor-mediated endocytosis (RME) system in a lot of cell types, and needs the different cover of exploitation target ligands.In the method, give this carrier cell specificity by the part that carrier is connected to selectively targeted cell surface receptor or label.Behind the specific binding, activate target cell RME system, make carrier/receptor complex internalization and digestion, some DNA payload is transported to nucleus and carries out gene expression.Some cell receptor can promote carrier directly to be absorbed into (Fernandez and Bailey, 1998 in the Cytoplasm by plasma membrane; The people such as Phelan, 1998; The people such as Rojas, 1998), but the most common approach that receptor-mediated macromole partially absorbs is endocytosis transportation (endocytic-trafficking) approach (Conner and Schmid, 2003).
There are some challenges about gene target being delivered to non-phagocytic mammalian cells: (i) break through the mammalian cell plasma membrane; (ii) exploitation makes the mechanism of delivery vector internalization; (iii) selection and grasp are used for the kind of the target ligands of targeting specific mammalian cell surface receptor; (iv) not exclusively degrade payload DNA and reach decomposition delivery vector in the cell; Reaching (v), payload DNA obtains discharging and being transported to mammalian cell Cytoplasm or nucleus.These challenges slightly change with the range gene delivery vector.Although carried out thorough research in this area, the detailed knowledge of related bioprocess is still not bery clear.
Also do not report any particle targeting non-phagocytic cell with bacterial cell or bacterial origin based on part, although may be because (a) can enter to non-phagocytic cell by the active phagocytic process, but the intracellular pathogen of the antibacterial that only lives can enter to non-phagocytic cell (that is, thinking that entering non-phagocytic cell is to order about the active phagocytic process of process by the multicomponent energy that needs that the bacterial pathogens of living is implemented) and (b) initiatively cell entry will refuse such as the passive processes such as receptor-mediated endocytosis based on part.Therefore, the bacterial cell that has killed does not participate in initiatively cell entry, and opposite with its natural tropism, live bacterial cell can not be drawn towards required non-phagocytic cell.Even the inactive particle of the bacterial cell that uses the targeting part to make to have killed or bacterial origin can endocytosis, the effective delivery of gene of expectability the method not.On the contrary, can expect endosome will degrade nonactive cell or particle, so that it is invalid as gene delivery vector.Only thinking at present thus that pathogenic bacterium can be expressed in the facultative cell of living makes it escape the protein of this endosome film.
Up to now, do not exist confirmed can be effectively with the antibacterial minicell carrier targeting non-phagocytic mammalian host cell method of delivery of gene payload thus.Although known road variety carrier targeting technology is taked wherein anyly can't cause that successful minicell target gene sends simply with expecting.This is to send owing to the biotic factor that is unique this scope can affect genes of interest the range gene delivery vector.
Therefore, need to be with the method for antibacterial minicell carrier specificity ground targeting non-phagocytic mammalian cells.
Summary of the invention
For reaching these and other requirement, one aspect of the present invention provides the target gene delivering method, it comprises makes bispecific part and following cells contacting: (i) be derived from the minicell of antibacterial, it contains the therapeutic nucleic acids sequence and reaches (ii) non-phagocytic mammalian cells.The two all has specificity to part to minicell surface composition and non-phagocytic mammalian cells surface composition.Mammalian cell swallows up minicell as a result, then produces the expression product of therapeutic nucleic acids sequence.Contacting between minicell and the mammalian cell can be in external or body.
The present invention is provided for the bispecific part with minicell carrier targeting non-phagocytic mammalian host cell equally.This bispecific part can be polypeptide or saccharide, and can comprise antibody or antibody fragment.In preferred embodiments, this bispecific part has and carries specific the first arm of minicell surface texture tool of antibacterial and carry specific the second arm of non-phagocytic mammalian cells surface texture tool.The surface texture of the minicell that ligand binding is required is the O-polysaccharide component of lipopolysaccharide.The required mammalian cell surface structure of ligand binding is receptor, preferably the receptor of the endocytosis of those energy activated receptor mediations.
The present invention provides a kind of compositions on the other hand, and it comprises that (i) contains the minicell that is derived from antibacterial of therapeutic nucleic acids and the bispecific part that (ii) can be combined with minicell surface composition and non-phagocytic mammalian cells surface composition.
Another aspect of the invention provides the minicell that is derived from antibacterial and the purposes of bispecific part in the preparation medicine that contains therapeutic nucleic acids, and this medicine is used for treating by it being given cell, tissue or organ the method for disease or change characteristic.This class medicine is used for by increasing required protein expression or function or treating various diseases and disease by the expression or the function that suppress destination protein matter.For example, the disease of intending treatment herein can be cancer, or acquired disease, for example AIDS, pneumonia, emphysema or the disease that caused by congenital error of metabolism, and for example the capsule fibroid becomes sick.As selection, but treatment influencing characterisitic, for example fertility or the immunne response relevant with allergen or infectant.
The accompanying drawing summary
Figure 1 shows that with non-targeted minicell contrast human androgen receptor-targeting restructuring minicell is introduced effective internalization of human prostate cancer LNCaP cell.Implement as described in Example 1 this process, come observed result by confocal microscope.The immunofluorescence dyeing of the image of all demonstrations all uses anti-Salmonella typhimurium (S.typhimurium) LPS monoclonal antibody specific then to use Alexa Fluor 594-to implement in conjunction with sheep anti-mouse igg (H+L) antibody.Shown in each figure be that differential interference differs the overlapping of (DIC) and red fluorescence image.(A) do not use the contrast LNCaP cell of minicell transfection.Carrying out not observing red fluorescence after the Salmonella typhimurium LPS dyeing.(B) be total to the incubation poststaining with non--targeting minicell transfection LNCaP cell and at 16 hours.Can be observed few background red fluorescence point.(C) with targeting minicell transfection LNCaP cell and at 16 hours poststainings.In the Cytoplasm of most cells, show red fluorescence, in black white image, represent with light gray.(D) be total to the incubation poststaining with non--targeting minicell transfection LNCaP cell and at 24 hours.Can be observed few background red fluorescence point.(E) with targeting minicell transfection LNCaP cell and at 24 hours poststainings.The result is presented in the Cytoplasm of most cells strong red fluorescence (light gray in the image).(F) identical with (E) but show single transfectional cell with higher enlargement ratio.Whole rubescent color fluorescence of Cytoplasm (light gray) almost.Listed the scale of each image.
Figure 2 shows that with non--targeting minicell contrast EGF receptor-targeting restructuring minicell is introduced the intracellular effective internalization of human breast cancer MDA-MB-468.Implement as described in Example 2 this process, come observed result by confocal microscope.Then the immunofluorescence dyeing of the image of all demonstrations all uses Alexa Fluor594-to implement in conjunction with sheep anti-mouse igg (H+L) antibody with anti-mouse typhus LPS monoclonal antibody specific.Shown in each figure be the overlapping of DIC and red fluorescence image.(A) do not use the contrast MDA-MB-468 cell of minicell transfection.Carrying out not observing red fluorescence after the Salmonella typhimurium LPS dyeing.(B) be total to the incubation poststaining with non--targeting minicell transfection MDA-MB-468 cell and at 24 hours.Can be observed few background red fluorescence point.(C) with targeting minicell transfection MDA-MB-468 cell and at 24 hours poststainings.Show red fluorescence (the light gray zone in the black white image) in the Cytoplasm of most cells surface and some cells.(D) identical with (C) but show single transfectional cell with higher enlargement ratio.The result is identical with (C).(E) identical with (D) 36 hours poststainings except cell.The result is presented in the Cytoplasm of most cells strong red fluorescence (light gray in the image).Listed the scale of each image.
Figure 3 shows that with non--targeting minicell and compare Her2/neu receptor-intracellular effective internalization of targeting restructuring minicell introducing human ovarian carcinoma SKOV-3.Implement as described in Example 3 this process, come observed result by confocal microscope.Then the immunofluorescence dyeing of the image of all demonstrations all uses Alexa Fluor 594-to implement in conjunction with sheep anti-mouse igg (H+L) antibody with anti-mouse typhus LPS monoclonal antibody specific.Shown in each figure be the overlapping of DIC and red fluorescence image.(A) do not use the contrast SKOV-3 cell of minicell transfection.Carrying out not observing red fluorescence after the Salmonella typhimurium LPS dyeing.(B) be total to the incubation poststaining with non--targeting minicell transfection SKOV-3 cell and at 36 hours.Can be observed few background red fluorescence point.(C) with targeting minicell transfection SKOV-3 cell and at 36 hours poststainings.Show red fluorescence (the light gray zone in the black white image) in the Cytoplasm of most cells.(D) identical with (C) but with higher enlargement ratio.The result is identical with (C).(E) show that divided by higher enlargement ratio several extracellulars are identical with (C).The result is presented in the Cytoplasm of most cells strong red fluorescence (light gray in the image).Listed the scale of each image.
Figure 4 shows that with the EGFR-targeting minicell that carries coding viral hepatitis Type B surface antigen plasmid the efficient of gene delivery to human breast carcinoma (MDA-MB-468) cell.(A) show the flow cytometry result of the fluorescence intensity of cell when carrying out following the processing: (i) with anti-HBsAg MAb then with phycoerythrin (PE)-in conjunction with secondary antibody (anti-mouse IgG) MAb; (ii) then use anti-HBsAg MAb and PE-in conjunction with anti-mouse IgG MAb with non--targeting minicell; (iii) then use anti-HBsAg MAb and PE-in conjunction with anti-mouse IgG MAb with non-specific targeting minicell; And (iv) EGFR-targeting minicell then with anti-HBsAg MAb and PE-in conjunction with anti-mouse IgG MAb.(B) show with EGFR-targeting minicell
HBsAgThe Laser Scanning Confocal Microscope result (ii and iii) that gene is effectively sent and recombinant HBsAg is expressed in the MDA-MB-468 cell after the transfection.The recombinant HBsAg protein of strong red fluorescence (in black white image, showing take light gray) as then showing in conjunction with anti-mouse IgG MAb with Alexa Fluor 594-with anti-HBsAg MAb in the cell.With non-specific targeting minicell
HBsAgThe control cells of transfection (i) only shows some background red fluorescence points.
Figure 5 shows that by the treatment of targeting restructuring minicell to human breast cancer xenograft in the nude mice.In nude mice, set up breast carcinoma xenograft (referring to embodiment 5), and carry out tumor inner therapeutic with the targeting restructuring minicell that carries plasmid pORF5-HSV1tk::Sh ble.The following tumor xenogeneic graft that carries out is treated: (the 1st group, matched group) tumor is not accepted any treatment; (the 2nd group, matched group) then treats tumor with 2 dosage GCV with non--targeting restructuring minicell [M-HSVtk]; (the 3rd group, matched group) is with targeting minicell [TM-HSVtk] the treatment tumor of recombinating; (the 4th group, matched group) uses bi-specific antibody (BsAb; The anti-human class EGF receptor-specific of anti-mouse typhus LPS/) then with 2 dosage GCV treatment tumor; (the 5th group, experimental group) recombinates minicell [TM-HSVtk] then with 1 dosage GCV treatment tumor with targeting; (the 6th group, experimental group) recombinates minicell [TM-HSVtk] then with 2 dosage GCV treatment tumor with targeting.Being depicted as under the X-axis in which day gives concrete group various treatments.
Figure 6 shows that by the minicell targeting of will recombinating and cross the EGF receptor of expression to the treatment of human breast cancer xenograft in the nude mice.In nude mice, set up breast carcinoma xenograft (referring to embodiment 6), and carry out tumor inner therapeutic with the targeting restructuring minicell that carries plasmid pORF5-HSV1tk::Sh ble.The following tumor xenogeneic graft that carries out is treated: (the 1st group, matched group) do not treat; (the 2nd group, matched group) non--and targeting restructuring minicell is [non--T-M
HSVtk] then with 2 dosage GCV; (the 3rd group, matched group) non--and targeting restructuring minicell is [non--T-M
HSVtk]; (the 4th group, matched group) bi-specific antibody (BsAb; The anti-human class EGF receptor-specific of anti-mouse typhus LPS/) then with 2 dosage GCV; (the 5th group, experimental group) targeting restructuring minicell [T-M
HSVtk]; (the 6th group, experimental group) is with 10
8Individual targeting restructuring minicell [T-M
HSVtk] then with 2 dosage GCV; And (the 7th group, experimental group) is with 10
9Individual targeting restructuring minicell [T-M
HSVtk] then with 2 dosage GCV.Being depicted as under the X-axis in which day gives concrete group various treatments.Solid triangle represents minicell or Antybody therapy, and hollow triangle represents the GCV treatment.
Figure 7 shows that by the treatment of the low HER2/neu receptor of expressing of the minicell targeting of will recombinating to human breast cancer xenograft in the nude mice.In nude mice, set up breast carcinoma xenograft (referring to embodiment 5), and carry out tumor inner therapeutic with the targeting restructuring minicell that carries plasmid pORF5-HSV1tk::Sh ble.With being administered to 8 groups of mices in the restructuring small cell tumor.The following tumor xenogeneic graft that carries out is treated: (the 1st group, matched group) do not treat; (the 2nd group, matched group) non--and targeting restructuring minicell is [non--T-M
HSVtk] then with 2 dosage GCV; (the 3rd group, matched group) is [non--T-M with non--targeting restructuring minicell
HSVtk]; (the 4th group, matched group) bi-specific antibody (BsAb; The anti-human class HER2/neu receptor-specific of anti-mouse typhus LPS/) then with 2 dosage GCV; (the 5th group, experimental group) targeting restructuring minicell [T-M
HSVtk]; (the 6th group, experimental group) is with 10
8Individual targeting restructuring minicell [T-M
HSVtk] then with 2 dosage GCV; (the 7th group, experimental group) is with 10
9Individual targeting restructuring minicell [T-M
HSVtk] then with 2 dosage GCV; And (the 8th group, experimental group) is with 10
9Individual targeting restructuring minicell [T-M
HSVtk] then with 2 dosage GCV intratumor injections.Being depicted as under the X-axis in which day gives concrete group various treatments.Solid triangle represents minicell or Antybody therapy, and hollow triangle represents the GCV treatment.
DESCRIPTION OF THE PREFERRED
The inventor has found to use the bispecific part with antibacterial minicell carrier targeting non-phagocytic mammalian host cell.This class host cell resists usually that minicell adheres to and endocytosis in the body, but by the bispecific part its can be easy to accept the minicell delivery vector in conjunction with and internalization.
Inventor's internalization minicell of finding again fully to degrade can discharge recombinant plasmid dna.This point is astonishing, because the non-phagocytic mammalian cells nature are not carried the aggressivity intracellular region chamber as the phagolysosome, phagolysosome mainly is present in immune system cell, for example engulfs macrophage.
Another surprisingly the inventor find equally the minicell of antibacterial can cause recombiant plasmid from nonphagocytic late period endosome escape.Because of the chromosome of minicell without the parental generation antibacterial of life and shortage coding endosome in late period and dissolving phagosome memebrane protein outside this is unexpected.In fact, usually generally acknowledge always only have through being designed for the dissolving lysosome membrane and bacterial pathogens could be with gene delivery to non-full-time phagocyte (recently by the people such as Grillot-Courvalin summary, 2002) in the facultative cell of the work of released dna in cell.For example, Listeria monocytogenes (Listeria monocytogenes) is expressed a kind of pore-forming cytolysin-Li Salmonella hemolysin O (by hly gene chromosome coding), it is considered to play an important role in dissolving endosome and phagosome film, by this so that recombinant DNA enters the infection cell Cytoplasm.Similarly, Fu Shi bacillus dysenteriae (Shigella flexneri) is considered to escape phagocytic vacuole by dissolving phagosome film equally.
The inventor confirms that further the recombination that minicell mediates effectively is delivered to the non-phagocytic cell nucleus relates to the plasmid copy number that is carried by minicell.So, the minicell that carries high copy number plasmid (every minicell surpasses 60 plasmid copies) can make gene effectively be delivered to non-phagocytic cell, yet the minicell efficient of carrying medium copy (11 to 60 of every minicells) or low copy (1 to 10 of every minicell) number plasmid is lower.
In addition, the inventor has confirmed that the minicell number that gene delivery efficient and pinocytosis enter in the endosome is relevant.Therefore, non-ly engulf target cell and demonstrate and in each endosome, swallow up more minicells what cell surface carried high expressed receptor (for example EGF receptor on some mankind mastopathy cell surface) and bispecific part targeting, usually surpass 10, cause the recombination high-efficiency delivery to the nucleus of this cell.These results suggest when the recombinant DNA as many as adequate remedy endosome of interior body burden during by the degraded loss from late period chance that endosome is escaped recombinant DNA increased.The same mammalian cell surface receptor of crossing expression at cell surface by use that shows of this class result makes a large amount of minicells of each endosome endocytosis can reach effectively sending of gene by this.
According to aforementioned discovery, the present invention by strengthen usually to minicell adhere to, endocytosis and the unresponsive target cell of gene delivery or organize medium and small cell transfecting efficient to enlarge and can use the minicell carrier to carry out the diseases range of gene therapy.Minicell targeting ability provides the safer more flexibly gene therapy system that reaches equally.
One aspect of the present invention provides the target gene delivering method, and it comprises allows bispecific part and following cells contacting: (a) be derived from the minicell of antibacterial, it contains the therapeutic nucleic acids sequence, and (b) non-phagocytic mammalian cells.The two all has specific bispecific part and facilitates minicell to be combined with mammalian cell to minicell and mammalian cell composition, so makes mammalian cell swallow up minicell, then produces the expression product of therapeutic nucleic acids sequence.
The inventor finds that the method can be widely used in the multiple non-phagocytic mammalian cells that usually is difficult to specific adsorption and endocytosis minicell.For example, the bi-specific antibody part of the anti-HER2 receptor of tool, anti-EGF receptor or antiandrogen receptor-specific can effectively be bonded to minicell various nonphagocytic each autoreceptor at the anti-O polysaccharide specificity of tool on the one arm and on other one arm.These cells comprise lung carcinoma cell, ovarian cancer cell, brain cancer cell, breast cancer cell, prostate gland cancer cell and skin cancer cell.In addition, effective combination is prior to the quick endocytosis minicell of each non-phagocytic cell.
The inventor's discovery is astonishing because before thought only have " sole duty " phagocyte (for example macrophage and neutrophilic leukocyte) can pinocytosis the so larger macromole particle (600 nanometers and larger) of bacteria-like cell.On the contrary, but think the only little abiotic macromole particle of pinocytosis of non-phagocytic mammalian cells, for example liposome (it is the 150-400 nanometer) and virus (it is about 65-80 nanosized).Referring to Bondoc and Fitzpatrick, 1998.The complete minicell that is derived from antibacterial that is used for inventor's research is about 400 nanometers of diameter.
The inventor finds that equally the recombinant DNA that minicell carries can pass through the non-phagocytic mammalian host cell expression.This class minicell is in case degraded in the endosome late immediately by pinocytosis.Yet some recombinant DNA that is carried by minicell is escaped the endosome film and is transported to the mammalian cell nucleus and makes its gene expression.This discovery is wondrous only had the facultative intracellular pathogen of living to carry toxic protein and the delivery of gene that can escape the endosome film because before thought.Referring to people such as Grillot-Courvalin, 2002.It is believed that the non-living body antibacterial or be derived from the minicell body of antibacterial and can not express the toxic protein that these are induced, expect that thus it is degradable in endosome, can not have any recombinant DNA to escape from endosome.
Therefore the present invention provides new method, its expansion can accept the scope of the mammalian cell of the minicell gene therapy by being derived from antibacterial.These methods all can be implemented in external and body.
Be used for part of the present invention and comprise any agent that is bonded to target cell surface composition and minicell surface composition.Preferred target cell surface composition is receptor, especially can mediate the receptor of endocytosis.This class part can comprise polypeptide and/or carbohydrate content.Antibody is preferred part.For example, the bi-specific antibody that carries the complete minicell surface composition that is derived from antibacterial and target mammalian cell surface composition dual specificity can be used for minicell efficient targeting target mammalian cell in external and body.Useful part comprises receptor, enzyme, binding peptide, fusion/chimeric protein and micromolecule equally.
Implement the selection of particular ligand at two main foundations: (i) specific binding to one or more domains on complete minicell surface and (ii) specific binding to one or more domains on target cell surface.Therefore, preferred part has and carries specific the first arm of complete minicell surface texture tool that is derived from antibacterial and carry specific the second arm of non-phagocytic mammalian cells surface texture tool.First and second arm all can be multivalence separately.Even be multivalence, preferably each arm is monospecific.
For being bonded to the minicell that is derived from antibacterial, an arm of expectation part is to being found in the O-polysaccharide component tool specificity of the lipopolysaccharide on the parental generation bacterial cell.Other minicell surface texture that can be used for ligand binding comprises the polypeptide that is exposed to cell surface and saccharide, pili (pilli), cilium (fimbrae) and the flagellum (flagella) on the adventitia.
For being bonded to target cell, an arm of part is to non-phagocytic mammalian surface composition tool specificity.This constituents comprises cell cortex protein, peptide and saccharide, and no matter whether it represents the characteristic of this cell.The cell surface receptor especially endocytosis person of those energy activated receptor mediations is the required cell surface composition of targeting.
For example, its can be by selecting the cell surface receptor motif on the required cell of specific binding part target tumor cell, metastatic cell, vascular cell (for example endotheliocyte and smooth muscle cell), pneumonocyte, nephrocyte, blood cell, medullary cell, brain cell, hepatocyte etc., or the predecessor of arbitrary selected cell.The cell surface receptor example comprises carcinoembryonic antigen (CEA), and it is crossed in most of colon and rectum carcinoma, breast carcinoma, pulmonary carcinoma, cancer of pancreas and gastrointestinal cancer and expresses (Marshall, 2003); Transfer protein receptor (HER-2, neu or c-erbB-2), its frequent mistake in breast carcinoma, ovarian cancer, colon cancer, pulmonary carcinoma, carcinoma of prostate and cervical cancer is expressed people such as (, 2000) Hung; EGF-R ELISA (EGFR), it crosses expression (people such as Salomon, 1995) at the various solid tumor camber that comprise breast carcinoma, head and neck cancer, nonsmall-cell lung cancer and prostate; Asialoglycoprotein receptor (Stockert, 1995); TfR (Singh, 1999); Silk presses down albumen (serpin) multienzyme complex receptor, and it is at liver cell expression people such as (, 1997) Ziady; Fibroblast growth factor acceptor (FGFR), it cross to express people such as (, 2002) Kleeff in pancreas pipeline adenocarcinoma cell; Vascular endothelial growth factor receptor (VEGFR), it is used for angiogenesis inhibitor gene therapy (people such as Becker, 2002 and the people such as Hoshida, 2002); Folacin receptor, its selectivity in 90% ovarian cancer is crossed expression (Gosselin and Lee, 2002); Cell surface glycocalyx (people such as Batra, 1994); Saccharide receptor (people such as Thurnher, 1994); And the polymerization immunoglobulin receptor, it is used for gene delivery to airway epithelial cell, and interesting aspect treatment lung disease (becoming sick such as the capsule fibroid) people such as (, 1997) Kaetzel.
Preferred part comprises antibody and/or antibody derivatives.Term used herein " antibody " comprises by producing the immunoglobulin molecules that immunogenic response obtains in external or the body.Term " antibody " comprises polyclone, monospecific and monoclonal antibody and antibody derivatives, for example single chain antibody fragments (scFv).Being used for antibody of the present invention and antibody derivatives can obtain by recombinant DNA technology equally.
Wild type antibody has four polypeptide chains, two identical heavy chains and two identical light chains.Two types of polypeptide chains all have constant region (it does not change or minimally changes) and variable region in same class antibody.The variable region is unique to a specific antibodies, and comprises the antigen binding domain of identification specificity antigenic determinant.The antigen binding domain district that major part is participated in antibodies directly be " complementary determining region " (CDRs).
Term " antibody " comprises antibody derivatives equally, for example keeps specific binding to the antibody fragment of antigenic capacity.This antibody-like fragment comprises Fab fragment (contains antigen-in conjunction with the territory and comprises light chain and part heavy chain fragment by the disulfide bond bridging), Fab ' (a kind of single antigen-in conjunction with the antibody fragment in territory of containing, the part heavy chain that it comprises Fab and passes hinge region), F (ab ') 2 (two Fab ' molecules that the intrachain disulfide bond by the heavy chain hinge region connects), bispecific Fab (one has the Fab molecule of two antigen binding structural domains, each can be directly from different antigenic determinants in conjunction with) and scFv (the single light chain of the antibody that connects together by amino acid chain and the variable antigen of heavy chain-in conjunction with determining area).
When antibody (comprising antibody fragment) consists of ligand moiety or all the time, is preferably the people source or is suitable for the mankind through improvement.So-called " humanized antibody " is well-known in the art.For example, referring to people such as Osbourn, 2003.It improves to reduce its antigenicity in the mankind by genetic manipulation and/or extracorporeal treatment.The method of humanized antibody is set forth (for example) in United States Patent (USP) the 6th, 639, and No. 055, the 5th, 585, No. 089 and the 5th, 530, in No. 101.In the simplest situation, the antigen-coupling collar of humanized antibody by will being called complementary determining region (CDRs) moves from mice mAb and receives IgG and form.Referring to people such as Jones, 1986; The people such as Riechmann, 1988; Reach the people such as Verhoeyen, 1988.Yet, produce the high affinity humanized antibody and usually need to shift one or more extra residues from the so-called framework region (FRs) of mice parent mAb.Several different humanization technology have equally been developed.Referring to people such as Vaughan, 1998.
The human antibodies that is different from " humanized antibody " can be used among the present invention equally.It has high affinity to antigen separately, usually obtains from extremely jumbo single chain variable fragment (scFvs) or Fab phage display library.Referring to people such as Griffiths, 1994; The people such as Vaughan, 1996; The people such as Sheets, 1998; The people such as de Haard, 1999; Reach the people such as Knappik, 2000.
Useful part comprises bispecific single-chain antibody equally, it typically is the recombinant polypeptide that the covalently bound extremely corresponding variable heavy chain of variable light chain part is partly formed by by linkers.Referring to United States Patent (USP) the 5th, 455, No. 030, the 5th, 260, No. 203 and the 4th, 496, No. 778.Same available other method of bi-specific antibody is made.For example, can create heteroconjugate by the chemistry not homospecific complete antibody of connection or antibody fragment.Referring to people such as Karpovsky, 1984.Yet this class heteroconjugate is difficult to repeat preparation, and it is large to be at least the twice of normal monoclonal antibody.Bi-specific antibody can be created by disulfide exchange equally, and it relates to enzymatic lysis and antibody fragment reconnects.Referring to people such as Glennie, 1987.
Because Fab and scFv fragment are unit price, it is usually to target structure tool low-affinity.Therefore, for increasing functional affinity, preferably from these compositions, make ligand design be dimer, trimer or tetramer conjugate.Referring to Tomlinson and Holliger, 2000; Carter, 2001; Hudson and Souriau, 2001; Reach the people such as Todorovska, 2001.This class conjugate structure can by chemistry and/or genetic engineering is crosslinked be created.
Preferred bispecific part of the present invention is each end monospecific, namely at one end to minicell single composition tool specificity and at the other end to the single composition tool of target cell specificity.Part can be at one end or two ends multivalence all, for example, and with so-called diploid, triplet and quaternary body form.Referring to Hudson and Souriau, 2003.Diploid is that it produces two Fv binding sites by two non-covalent bivalent dimers that are connected to form of scFv.Similarly, triplet forms the trivalent trimer by three scFv and produces, and obtain three binding sites, and quaternary body forms the generation of tetravalence tetramer by four scFv, obtains the four combinations site.
Several to the specific humanization of receptor tool, the mankind and mouse monoclonal antibody on the mammalian cell and fragment thereof its human treatment's purposes that gone through, this list increases sharply.Referring to Hudson and Souriau, 2003.The antibody example that this kind can be used for forming bispecific part one arm is to HER2 tool specificity: Trastuzumab (Herceptin
TM); Herceptin (Trastuzumab).
Antibody variable region can merge with the protein domain of broad range equally.Not only increase quality but also promote dimerization with human immunoglobulin domain (for example IgG1 CH3) fusion.Referring to people such as Hu, 1996.Can increase effector functions with human Ig hinge-Fc zone fusion.Can promote polymer equally with the protein domain fusion of polymer protein.For example, merge to produce miniantibody with lacking scFv with short both sexes flight.Referring to Pack and Pluckthun, 1992.The domain (such as fos/jun) that forms the protein of heterodimer can be used for producing two special moleculars (people such as Kostelny, 1992), perhaps, all engineering strategy (such as " knobs into holes ") design forming heterodimer people such as (, 1996) Ridgway can be passed through in the dimeric structure territory.At last, can select the fusion rotein companion that not only provides polymerization but also other function is provided, for example streptavidin.Referring to people such as Dubel, 1995.
Minicell of the present invention be escherichia coli or other bacterial cell without kernel form, it causes by harmony of destroying DNA separate during the cell division dyad.The protokaryon Chromosomal duplication links to each other with normal dyad, and it participates in the medium cell barrier film and forms.For example, min gene in escherichia coli (for example minCD) sudden change can be eliminated during cell division the cell summit every film formed inhibition, causes normal-sub cell and seedless minicell to produce.Referring to de Boer1992; Raskin and de Boer, 1999; Hu and Lutkenhaus, 1999; Harry, 2001.Minicell is different from the vesicles of other spontaneous generation and release under some environment, and the latter compares with minicell, resets or episome gene expression not due to specificity heredity.For carrying out the present invention, the complete cell wall (" complete minicell ") of expectation minicell tool.
Except the min operator mutation, seedless minicell can be reset or the rear generation of sudden change (for example bacillus subtilis (B.subtilis) divIVB1) every film formed other heredity in various impacts equally.Referring to Reeve and Cornet, 1975; The people such as Levin, 1992.Minicell can form behind the gene expression dose that disturbs the protein that participates in cell division/chromosome separation equally.For example, crossing expression minE causes polarity division and minicell to form.Similarly, the less minicell of chromosome can be produced by the chromosome separation defective, for example, smc sudden change in bacillus subtilis people such as (, 1998) Britton, (the people such as Ireton of spoOJ disappearance in the bacillus subtilis, 1994), parC sudden change (Stewart and D ' Ari, 1992) in mukB sudden change in escherichia coli people such as (, 1989) Hiraga and the escherichia coli.Gene outcome can transly provide.For example, when high copy number plasmid was crossed expression, CafA can improve cell division rate and/or inhibition to be copied the after stain colour solid and distributes people such as (, 1994) Okada, caused formation (people such as Wachi, 1989 of chain type cell and seedless minicell; The people such as Okada, 1993).Minicell can be from any Gram-positive or the preparation of gram negative bacteria cell derived.
Minicell of the present invention contains transcribed and/or translates to produce the nucleic acid molecules of required product.For this description, this class nucleic acid molecules is categorized as " therapeutic nucleic acid molecule ".In certain embodiments, this is transcribed and/or translation product plays a part to improve in cell, tissue or organ or treats in addition disease or change characteristic.General therapeutic nucleic acid is present on the interior plasmid of minicell.
The product that the therapeutic nucleic acid molecule coding is wished generation, for example function RNA (for example antisense RNA, ribose ribozyme, siRNA or shRNA) or peptide, polypeptide or protein.For example, the hormone of interested hereditary material codified tool therapeutic value, receptor, enzyme or (many) peptides.These class methods can cause that not the extrachromosomal replication of transient expression, transfer replication (for example episome) of the transfer DNA of integrating and expression or transfer material are integrated among the host cell gene group DNA.
Transcribing or translating of particular treatment nucleic acid molecules can be used for treating cancer or acquired disease, for example AIDS, pneumonia, emphysema or the disease relevant with congenital error of metabolism, for example capsule fibroid change disease.Transcribing or translate equally of therapeutic nucleic acids can realize the sterillization of practising contraception, and comprises the contraception sterillization of wild animal.Inflammatory disease allergen mediation and the infectant mediation can be offset by giving therapeutic nucleic acid molecule of the present invention equally, after this therapeutic nucleic acid molecule is expressed in the patient, affects the immunne response relevant with separately allergen and infectant.Therapeutic nucleic acid molecule can have expression product equally, maybe can have the downstream product of expression product post translational modification, and it reduces and transplants relevant immune sequela, or helps lend some impetus to tissue growth and regeneration.
Therapeutic nucleic acid molecule can be the normal counter pair of gene, this gene expression plays Effects of Anomalous or exists with abnormal level in morbid state protein, for example, following is exactly this situation: become cystic fibrosis cross-film conduction instrumentality in the disease (people such as Kerem, 1989 in the capsule fibroid; The people such as Riordan, 1989; The people such as Rommens, 1989); Betaglobulin in the sickle cell disease and the alpha-globulin in the thalassemia, betaglobulin and gamma globulin.Therapeutic nucleic acid molecule can have antisense RNA transcript or siRNA as mentioned above.Therefore, be characterized as alpha-globulin and can alleviate by gene therapy its complete minicell that contains the plasmid of having integrated the antisense RNA transcript relative with target sequence alpha-globulin mRNA through design used according to the invention above the β-thalassemia of the excessive formation of betaglobulin.
In treatment of cancer, be applicable to the sequence that therapeutic nucleic acid molecule of the present invention can have corresponding to or be derived from the gene relevant with suppressing tumor (for example gene of p53 gene, retinoblastoma gene and codes for tumor necrosin).Can treat widely various solid tumor-cancers, papillary tumor and wart according to the present invention by the method.The representative cancer of this respect comprises colon cancer, carcinoma of prostate, breast carcinoma, pulmonary carcinoma, skin carcinoma, hepatocarcinoma, osteocarcinoma, ovarian cancer, cancer of pancreas, the brain cancer, head and neck cancer and lymphoma.Illustrative papillary tumor is squamous cell papilloma, papilloma of choroid plexus and Laryngeal papilloma.The Verrucosis example is reproduction wart, the plantar wart, epidermodysplasia and pernicious wart.
Therapeutic nucleic acid molecule of the present invention can comprise the dna fragmentation that coding is converted into the non-activity prodrug enzyme of one or more cytotoxicity metabolite equally, in case introduce like this this prodrug in the body, will force the target cell (perhaps also together with adjacent cells) in the effect to commit suiside.Before this " suicide gene " (it can be inhuman source or people source) clinical and clinical practice summarize in the people (2002) such as the people (2000) such as Spencer (2000), Shangara and Yazawa.Exemplary inhuman source suicide gene is the gene of those HSV-thymidine kinases (tk) of encoding respectively, cytosine deaminase (CDA)+uracil phosphoribosyl transferring enzyme, xanthine-guanine ribose phosphate-transferring enzyme, nitroreductase (NTR), purine nucleoside phosphorylase (PNP, DeoD), Cytochrome P450 (CYP4B1), CPG2 (CPG2) and D-AAO (DAAO).People source suicide gene has the Carboxypeptidase A l (CPA) that encodes respectively, deoxycytidine kinase (dCK), Cytochrome P450 6 for example), the gene of LNGFR/FKBP/Fas, FKBP/ Caspase class and ER/p53.
Suicide-gene therapy can be applicable to treat AIDS.This strategy was tested, as long as the mammalian cell for the treatment of uses the suicide vector of expressing poisonous gene outcome once being infected by HIV at once.These carriers use HIV-1 regulating element (Tat and/or Rev) to induce poisonous gene expressions such as α-diphtheria toxin, diphtherotoxin, cytosine deaminase or interferon-' alpha ' 2 after infecting at HIV-1.Referring to people such as Curiel, 1993; The people such as Dinges, 1995; The people such as Harrison, 1992a; The people such as Harrison, 1992b; The people such as Ragheb, 1999.
Therapeutic nucleic acids of the present invention is contained on the plasmid in the minicell usually.This plasmid can contain the extra nucleic acid fragment that works as regulating element equally, for example promoter, terminator, enhancer or signal sequence, and it operationally connects together with the therapeutic nucleic acids fragment.Suitable promoter can be depicted as tissue-specific or even for tumour-specific such as therapeutic domain.
It is " tissue-specific " when a promoter preferentially activates in a particular organization, and it effectively drives the expression of the structure sequence that is operatively connected in target tissue thus.For example, the kind of tissue-specific promoter comprises: respectively for albumin and α
1-antitryptic hepatocyte-specificity promoter; Elastoser I gene-controlled area, it activates in pancreatic acinar cell; The insulin gene control zone, it activates in pancreatic beta cell; MMT virus control district, it activates in testis, mammary gland, lymph and mastocyte; Myelin basic protein plasmagene control zone, it activates in the brain oligodendroglia; And the gonadotropin releasing hormone gene-controlled area, it activates in hypothalamus cells.Referring to people (1986) such as the people (1987) such as people (1986), the Readhead such as the people (1984) such as people (1987), the Swift such as people (1987), the Kelsey such as people (1985), the Pinkert such as the people such as Frain (1990), Ciliberto, MacDonald (1987), Hanahan (1985), Leder and Mason.
Have equally in some tumor cell or in the preferential promoter of expressing of tumor cell itself, it can be used for treating various cancers according to the present invention.To the specific promoter kind of cancer cell for example: tryrosinase promoter, its targeting melanoma; The MUC1/Df3 promoter, its targeting breast carcinoma; Heterozygosis myoD enhancer/SV40 promoter, its targeted expression rhabdomyosarcoma (RMS); Carcinoembryonic antigen (CEA) promoter, it is to CEA express cell (for example colon cancer cell) tool specificity; And hexose kinases II type gene promoter, its targeting nonsmall-cell lung cancer.Referring to people (1999) such as the people such as Hart (1996), Morton and Potter (1998), Kurane and Katabi.
Can affect the secretion of expression product or expression product is positioned specific cellular compartment with signal sequence according to the present invention.Therefore, the therapeutic polynucleotide sequence molecule of sending by complete minicell can comprise the signal sequence that is in the suitable reading frame, so that the purpose expression product is secreted, affect by this peripheral cell consistent with selected treatment example in eat cell or its offspring.Exemplary signal sequence comprises that the terminal secretion sequence of hemolysin C-(is set forth in United States Patent (USP) the 5th, 143, in No. 830), the BAR1 secretion sequence (is disclosed in United States Patent (USP) the 5th, 037, in No. 743) and the signal sequence of zsig32 polypeptide part (be set forth in United States Patent (USP) the 6th, in 025, No. 197).
Plasmid in the minicell of the present invention can contain the report element equally.The report element can not be given phenotype or the characteristic that its recombinant host is convenient to detect by the polypeptide that the host produces by coding usually, and it is in case express and can detect by histology or original position analysis (for example animal imaging).For example, according to the present invention, the report element codified of being sent by complete minicell produces the protein of tool colourity or change in fluorescence in the host cell of eating, and it can be by the original position analyzing and testing, and has quantitatively or the function of sxemiquantitative transcriptional activity.This exemplary proteinoid is lipase, phosphatase, protease and other enzyme, and its activity form produces detectable chromophore or fluorogen.
Preferred example is escherichia coli beta galactosidase (it affects change color by the former substrate indole-β of cracking indigo-D-galactoside) and luciferase (its oxidation long-chain aldehyde (luciferase of antibacterial) or heterocyclic carboxylic acid (fluorescein) are simultaneously luminous).Equally usefully encode the in this article report element of green fluorescent protein (GFP) of Jellyfish (Aequorea victoria), its such as the people such as Prasher (1995) elaboration.(polynucleotide sequence of 238 the amino acid whose GFP apoproteins of encoding is disclosed with the technology of GFP domain-specific by the PCT application WO 095/21191 of two announcements, it contains from 65 amino acids to 67 amino acids the chromophore that forms) and WO 095/21191 (cDNA that modifies A.victoria GFP apoenzyme peptide is disclosed, it provides tool to change the peptide of photoluminescent property) and the people (1994) such as Heim (report one sudden change GFP, it is characterized by the exciting light amplitude improve 4-to-6-doubly) illustrate.
Another type report element with so that the expression product that the minicell of recombinating can fight toxins is relevant.For example neo gene protection host resists the toxic level of antibiotic G418, and the gene of coding dihydrofolate reductase provides the resistance of anti-methotrexate, and chloramphenicol acetyltransferase (CAT) gene provides the chloramphenicol resistance resistance.
Other comprises that with the gene of element of giving a report those can transform host's minicell to express the gene of distinguishing cell surface antigen, for example, virus envelope albumen, for example HIV or herpes gD, it is easy to detect by immunoassay.
Target cell of the present invention comprises introduces any cell in it with exogenous nucleic acid molecule.(nucleic acid molecules that meaning should be carried in minicell when exogenous nucleic acid molecule is used " introducing " is delivered to target cell.) required target cell is characterized as the express cell surface receptor, in case this receptor and ligand binding promote endocytosis at once.Preferred target cell is non-phagocytic cell (meaning i.e. this cell under normal circumstances can not the bacterial digestion particle) and is mammalian cell.
The inventive method and compositions can be used for sending the multiple nucleic acids molecule, and it can be cDNA or RNA, also can be genomic DNA or RNA, and can be in justice or antisense orientation.According to the present invention, the nucleic acid molecules that is present in minicell can be rendered as plasmid, expression vector or other construction form, but can not be the genomic DNA that derives from the bacterial cell that produces minicell.Being applicable to the present inventor is DNA or the RNA sequence that needs from eucaryon, protokaryon or synthetic any phase of originating, and it can be translated and transcribe under the control of eukaryotic gene expression promoter, or uses and express in mammalian cell from the transactivation factor of host cell.
The inventive method can be in vivo or first in the external rear body (ex vivo) implement.For example, formerly in the interior method of external rear body, can remove target cell by biopsy from an experimenter (for example).Can select suitable part based on the knowledge to the cell surface receptor of being expressed by this target cell.The gene clone that plan is delivered to target cell enters in the suitable episome carrier DNA (for example plasmid), and changes the parent bacterial cell of complete minicell origin over to.The process that obtains minicell is well known in the art, such as among the PCT/IB02/04632 elaboration.Then carry the minicell of recombinant DNA by known method purification in this area, it is set forth among the PCT/IB02/04632.For example, then by external incubation in suitable culture medium with the purification minicell of bispecific ligand binding to this restructuring, unnecessary part is washed off from lotus has the minicell of part.Then allow the compositions of the complete minicell that comprises purification and bispecific part (it is by being attached to minicell to the specific arm of minicell surface composition tool) and target cell or external (for example, in tissue culture, as described in embodiment 1,2 and 3) or in vivo (as described in Example 4) contact.
Therefore, present invention resides in the method for implementing first external rear vivo gene treatment in the required non-phagocytic mammalian cells (it is not replied the gene therapy of minicell mediation under normal circumstances).Visual target cell of the present invention and therapeutic nucleic acids and be used for the treatment of various diseases and disease are increasing the expression of desired protein, with the expression of suppressor gene product or function etc.For example, transcribe or translate the particular treatment nucleic acid molecules and can be used for treating cancer or acquired disease, for example AIDS, pneumonia, emphysema or the disease relevant with proofreading and correct congenital error of metabolism, for example capsule fibroid change disease.Transcribe or translate therapeutic nucleic acids and can cause the sterillization of practising contraception equally, comprise wild animal contraception sterillization.Inflammatory disease allergen mediation and the infectant mediation can be offset by giving therapeutic nucleic acid molecule of the present invention equally, after this therapeutic nucleic acid molecule is expressed in the patient, affects the immunne response relevant with separately allergen and infectant.Therapeutic nucleic acid molecule can have expression product equally, maybe can have the downstream product of expression product post translational modification, and it reduces and transplants relevant immune sequela, or helps lend some impetus to tissue growth and regeneration.
The present invention relates to equally and external nucleic acid is transferred to selected cell type.This class shifts and is used for multiple purpose, for example creates to produce the cell of a large amount of selected protein (can gather in the crops subsequently this protein).
The present invention is provided for exogenous nucleic acid molecule is efficiently introduced the compositions of target non-phagocytic mammalian cells in the parties concerned.Said composition comprises minicell and (ii) the bispecific part that (i) is derived from antibacterial.This class minicell and part can be and be set forth in herein any.Therefore, minicell contains therapeutic nucleic acid molecule, and the bispecific part preferably can be in conjunction with minicell surface composition and target mammalian cell surface composition.
Basically recombinating the compositions that minicell and bispecific part form (that is comprising this minicell and part and the DNA-of the excessive interference said composition compositions of sending other composition of quality not) by the present invention can be with accepting carrier on one or more physiology or excipient is allocated in a usual manner.Injection preparation can be unit dosage form in ampoule or glass tube vial or multi-dose container, contain or do not contain extra antiseptic.This class preparation can be solution, suspension, the emulsion in oiliness or aqueous excipient, and can contain formula agent, for example suspending agent, stabilizing agent and/or dispersant.Suitable solution and receptor's blood etc. ooze, and illustrate by saline, RingerShi solution and glucose solution.As selection, compositions can be the lyophilized powder form redissolves with suitable medium, for example uses aseptic, apirogen water or normal saline.Compositions can be formulated as depot formulations equally.This class durative action preparation can be by implanting (for example, subcutaneous or intramuscular) or giving by intramuscular injection.
The various sites that the present composition can be imparted to mammalian body by all means to be reaching required therapeutical effect, itself or for local or send for system.For example, can give by per os, by preparation is applied in the body cavity, by sucking or be blown into, by in parenteral, intramuscular, intravenous, the portal vein, in the liver, in the peritoneum, subcutaneous, tumor or Intradermal implement to send.Giving mode and site decides on the target cell position.For example, the cystic fibrosis sexual cell can be sent targeting restructuring minicell by sucking efficient targeting.Similarly, neoplasm metastasis can be sent targeting restructuring minicell by intravenous and more effectively treated.The primary ovarian cancer can be sent targeting restructuring minicell by intraperitoneal and be treated.
The following example is intended to illustrate and provides and the present invention is more fully understood but not the present invention is limited to the embodiment that provides.
Originally experimental results show that contain carry anti-mouse typhus LPS and the specific Fab fragment of antiandrogen receptors bind bi-specific antibody can in conjunction with and enter known in cell surface is crossed the prostate gland cancer cell of expressing androgen receptor through the minicell that receptor mediation internalization is derived from mouse typhus.
Transform the previous Salmonella typhimurium minCDE-mutant (patent application case PCT/IB02/04632) that produces with recombiant plasmid pORF5-HSV1tk::Sh ble (Invivogen, San Diego, CA, USA).This plasmid is the mammalian gene expression carrier of expressing HSV1tk::Sh ble fusion gene under EF-1 α/eIF4g hybrid promoter control.HSV1tk is the suicide gene from herpes simplex 1 type virus (HSV1), and coding thymidine kinase this kind of enzyme, and this enzyme can be converted to ganciclovir-monophosphate (GCV-MP) with prodrug guanosine analogue ganciclovir (GCV).Then by interior living kinases the latter is converted to diphosphonic acid and triphosphoric acid form.The GCV-triphosphoric acid lack deoxyribose 3 ' OH and to the DNA chain extension requisite 2 ' and 3 ' carbon between key.The GCV-triphosphoric acid is integrated and to be caused that the DNA chain crosses early stopping and cause apoptosis as a result.Therefore it is responsive to ganciclovir that HSV1tk expresses the mammalian cell that makes transfection, and be the most widely used single commit suiside one of strategy (Singhal and Kaiser, 1998) of gene therapy for cancer.Make up wherein by with Restriction Enzyme NcoI and NheI cracking pORF5-HSV1tk::Sh ble plasmid with T4DNA polymerase blunt end site and reconnect the control plasmid that this plasmid is deleted HSV1tk::Sh ble fusion gene.NcoI and NheI site are unique site and at HSV1tk::Sh ble fusion gene flank in pORF5-HSV1tk::Sh ble plasmid.The plasmid that is called pORF5-HSV1tk that obtains is transformed in the Salmonella typhimurium minCDE-mutant equally.
Use such as the described gradient centrifugation of international application PCT/IB02/04632/thread shaping/filter/remove restructuring minicell that endotoxic program purification carries this class plasmid.
By resisting mouse typhus lipopolysaccharide (Biodesign, Saco, Maine, USA) and antiandrogen receptor mouse monoclonal antibody (IgG; Abcam, Cambridge, UK) the recombinant protein A/G that is connected to the Fc fragment purification of each monoclonal antibody makes up bi-specific antibody, and this program is as follows in brief.
Recombinant protein A/G (Pierce Biotechnology with purification, Rockford, IL, USA) being diluted to final concentration in the pure binding buffer liquid of immunity (Pierce Biotechnology) is 100 ug/ml, and in 4 ℃ allow 0.5 ml soln with contain anti-Salmonella typhimurium LPS (Research Diagnostics Inc., Flanders, NJ, USA) and anti-human class androgen receptor (Abacam, Cambridge, UK) aqueous premix of each 20 ug/ml of monoclonal antibody is incubated overnight.Then will not be bonded to following the removing of unnecessary antibody of a-protein/G.The gentle mixing
Protein G solution is (coated to the recombinant protein G on magnetic particle surface with covalent coupling
[2.8 microns]; Dynal Biotech, Oslo, Norway), 100 microlitre solution are transferred to the eppendorf centrifuge tube.Place Dynal MPC-S (magnetic particle concentrator, S type) to fix this beadlet, to discard supernatant this pipe.With this class beadlet Eddy diffusion in 0.5 milliliter of washing liquid that contains Na-phosphate buffer (pH 5.0).Repeat the fixing and washing step of beadlet three times.The solution that will contain a-protein/G-bi-specific antibody complex is added to beadlet and mixed incubation 40 minutes in room temperature is gentle.The eppendorf centrifuge tube is placed on the MPC-S platform with fixing beadlet, remove a-protein/G-bi-specific antibody complex with pipette.This step has been removed unconjugated unnecessary monoclonal antibody from solution, and provides and carry the solution that is connected to the bi-specific antibody of a-protein/G by its Fc fragment.
10
10Individual restructuring minicell and a-protein/G-bi-specific antibody in room temperature incubation 1 hour with antibody by its coated this class minicell in anti-LPS Fab zone.
Prostate gland cancer cell LNCaP (ATCC, Rockville, MD, USA) is grown in being supplemented with 10%FCS and antibiotic RPMI 1640 culture medium in the T-75 bottle fully and merges.In the T-25 bottle, merge this cell that goes down to posterity with 50%.Spend the night adhere to after, upgrade culture medium, in one bottle, add 10
7The individual restructuring minicell (non--targeting restructuring minicell) that carries plasmid pORF5-HSV1tk::Sh ble, and in another bottle, add 10
7Individual same but carry the minicell (targeting restructuring minicell) of the bi-specific antibody that is attached to cell surface.Minicell is 100: 1 to the ratio of prostate gland cancer cell.Transfectional cell is at 5%CO
2Reach incubation 16 in 37 ℃ of incubators, wash 4 times (each 5 milliliters) with the slight jolting of fresh 1x DulbeccoShi culture medium after 24 and 36 hours.Use the trypsin acting all cells, then the coverslip of 13 millimeters thick goes down to posterity (each time point is done three repetitions) in 24 orifice plates, and cell quantity is inferior the fusion.
With 4% paraformaldehyde the cell on the coverslip is fixed 30 minutes, and with the sealing of spending the night of 5% normal sheep serum, then use anti-Salmonella typhimurium LPS (1: 200; Biodesign, Saco, Maine, USA) monoclonal antibody dyeing.With in conjunction with Alexa Fluor 594 (1: 1000, red fluorescence; Exciting light 590 nanometers and utilizing emitted light 617 nanometers; Molecular Probes, Eugene, OR, USA) goat anti-mouse igg show antibodies, observe by fluorescence confocal microscope (Fluoview, Olympus America, Melville, NY, USA).Collect fluorescence and differential image contrast (DIC) image, it is as shown in Figure 1 overlapping.
The result shows that putting non--targeting restructuring minicell in any analysis time can not be attached to the LNCaP prostate gland cancer cell or realize internalization (Figure 1B and 1D) in the LNCaP prostate gland cancer cell by specificity, and cell shows equally with the contrast non-transfected cell.All visuals field of analyzing all show faint background red fluorescence.In contrast, find targeting restructuring minicell strong adhesion to the LNCaP cell, deduction is to be bonded to the cell surface androgen receptor by the bi-specific antibody targeting.In addition, at 16 hours and 24 hours incubative time points, most of LNCaP cell demonstrated strong red fluorescence (Fig. 1 C, 1E and 1F) in the Cytoplasm of this class cell, and it indicates that minicell is by receptor-mediated endocytosis internalization.
The minicell mediation minicell that this results suggest is carried the bi-specific antibody that is attached to the surface efficiently is bonded to the cell surface receptor (being androgen receptor in above-mentioned example) that is present in mammalian cell, and the minicell that adheres to is by rapidly internalization of non-phagocytic mammalian cells (being prostate gland cancer cell in above-mentioned example).
The embodiment 1 proof anti-LPS of tool (minicell specificity) and the specific bi-specific antibody of antiandrogen receptors bind can be bonded to effectively by force the androgen receptor on the non-phagocytic mammalian cells (prostate gland cancer cell).In addition, its result proves that the receptors bind high efficiency causes the endocytosis of receptor-mediated restructuring minicell.The phenomenon tool universality that present embodiment proof is observed above, and the present invention and discovery are applicable to the various different endocytosis active acceptors on the different non-phagocytic mammalian cells.
More precisely, this experiment shows mankind mastopathy cell (MDA-MB-468, ATCC; The human breast epithelial cell; The bi-specific antibody of Fab fragment that non-engulfing) can be by carrying anti-mouse typhus LPS (minicell surface combination specificity) and anti-epidermal growth factor receptor (EGFR) binding specificity comes targeting.Cell line MDA-MB-468 cell is grown in embodiment 1 described tissue culture for prostate gland cancer cell.Except replacing outside the antiandrogen acceptor monoclonal antibody with monoclonal antibody against EGFR (Oncogene Research Products, Cambridge, MA, USA), this bi-specific antibody makes up as described in Example 1.Generate targeting and non-targeted restructuring minicell and be used for transfection MDA-MB-468 cell, as above-mentioned prostate gland cancer cell, 16 hours, 24 hours and 36 hour time cell is carried out Salmonella typhimurium LPS (minicell) dyeing.
The result shows that (Fig. 2) control cells and the cell of processing with non-targeted minicell only show blush background fluorescence (Fig. 2 A and 2B) at all time points, and the prompting minicell can not adhere to and the transfection non-phagocytic mammalian cells.In contrast, in the showed cell matter strong red fluorescence is arranged behind 24 hours incubations of the cell of processing with the targeting minicell, this fluorescence is increased to and covers more Multi-cytoplasm (Fig. 2 C-E) after 36 hours.This points out that bi-specific antibody can make minicell and the strong combination of MDA-MB-468 cell surface EGF receptor, and this combination causes receptor-mediated minicell endocytosis.
Embodiment 3. bi-specific antibody targeting minicell efficient in conjunction with and enter in the non-human ovarian cancer cell of engulfing through receptor mediation internalization
Equally, originally experimental results show that human ovarian cancer cell (SKOV-3, ATCC; Epithelial cell; The bi-specific antibody of Fab fragment that non-engulfing) can be by carrying human Her2/neu receptor (Serotec Inc., Raleigh, NC, the USA) binding specificity of anti-mouse typhus LPS (minicell surface combination specificity) and mouse-anti comes targeting.Known SKOV-3 cell is crossed expression Her2 receptor (people such as Salomon, 1995).This experiment is implemented as described in embodiment 1 and 2, and sample such as before carry out anti-LPS (red fluorescence) dyeing.
Result (Fig. 3) is similar to embodiment 1 and 2 resulting results.Contrast SKOV-3 cell and the cell of processing with non--targeting minicell only show faint background red fluorescence.
The above-mentioned minicell that experimental results show that efficiently is attached to non-phagocytic mammalian cells, for example human epithelium's cancerous cell.Present embodiment proof non-phagocytic mammalian cells has the intracellular mechanism of effect degraded large pinocytosis particle as minicell (400 nanometer diameter).Present embodiment shows that equally being wrapped in the interior plasmid DNA of minicell can escape degradation process in the cell, can escape the endosome film, enters Cytoplasm, enters nucleus and recombinant expressed.In fact, effectively delivery of gene is to non-phagocytic cell for minicell, and it shows that the present invention is applied as useful in-vitro transfection instrument.
Allow mankind mastopathy cell (MDA-MB-468) with carry the coding viral HbsAg (HbsAg; Aldevron, USA) non-targeted, the non-specific targeting of contrast and the experiment EGFR-targeting minicell incubation of plasmid.Make up non-specific targeting BsAb with hugeization of anti-cell virus (CMV) monoclonal antibody and anti-Salmonella typhimurium LPS Mab.Wash this class cell 4 hours, 8 hours, 16 hours, 24 hours and 36 hour time, fix with 4% paraformaldehyde, with 5% normal sheep serum/2%BSA sealing.Increase permeability of the membrane with the 1%Triton X-100 among the PBS, and with anti-HbsAg MAb (Aldevron, with dilution in 1: 100) process cell, then use Alexa Fluor 594-to process in conjunction with goat anti-mouse igg (Molecular probes was with dilution in 1: 1000).Express the cell of HbSAg protein with the Laser Scanning Confocal Microscope analysis.For measuring gene delivery efficient, use the Flow Cytometry cell.For carrying out facs analysis, process cell with anti-HBsAg Mab, then use phycoerythrin (PE)-replace Alexa Fluor 594 to process cells in conjunction with goat anti-mouse igg, because PE is more responsive than 594 pairs of facs analysis of Alexa Fluor.
The result shows that the gene delivery efficient of only having the generation of EGFR-targeting minicell is greater than 95% (Fig. 4 Aiv).After the transfection 16 hours (Fig. 4 Aiv) and subsequently time point observe recombinant protein expression (the shinny red fluorescence of cell; Fig. 4 Bii-iii), point out the significance level of recombinant protein in each cell.All control cells are display background red fluorescence point (Fig. 4 Bi) only.
These results are astonishing, because people and do not know that non-phagocytic cell has the intracellular mechanism of effective degraded large pinocytosis particle as minicell (400 nanometer diameter) and has the rigidity biomembrane.In addition, observe the high efficiency level with gene delivery to non-phagocytic mammalian cells (greater than 95%) outside unexpected.These results point out that the present invention is applied as useful in-vitro transfection instrument.High degree is delivered to non-phagocytic mammalian cells with specific gene also not have at present useful tool can reach so.
Embodiment 5. Mediated by Bi-specific Antibodies is with the human breast cancer xenograft in the female nude mouse of minicell targeting
Present embodiment proof carry coding HSVtk gene plasmid targeting restructuring minicell can so that mankind mastopathy cell's tumor xenogeneic graft of setting up in the female nude mouse in 6 ages in week disappear.
Make up as described in Example 1 bi-specific antibody except replacing with anti-epidermal growth factor receptor (anti-EGFR) monoclonal antibody (Oncogene Research Products, Cambridge, MA, USA) outside the antiandrogen acceptor monoclonal antibody.This is because this xenotransplantation cell is the known mankind mastopathy cell MDA-MB-468 that expresses the EGF receptor that crosses at cell surface.Mice is available from Perth, the Animal resources center of WA, and all zooperies are according to management of laboratory animal and guide for use and carries out under the approval of animal Ethics Committee.Experiment is carried out in the toy field of the NSW of EnGeneIC Pty Ltd (Sydney, NSW, Australia) company agricultural approval.Cultivate as described in Example 2 the MDA-MB-468 mankind mastopathy cell, use No. 23 pins with the 1.5x10 in the 50 microlitre serum-free mediums
6Individual cell together with 50 microlitre somatomedin reproducibility matrigel (BD Biosciences, Franklin Lakes, NJ, USA) subcutaneous injections between the scapula of each mice.With digital electronic caliper (Mitutoyo, Japan are accurate to 0.001) a week measuring tumor 2 times, with formula length (centimetre) the x width
2(centimetre) X0.5=volume (cubic centimetre) calculating gross tumor volume.Implant rear 21 days gross tumor volumes and reach between 50 cubic centimetres and 80 cubic centimetres, mice is divided into six not on the same group at random, 12 every group.
Experimental design is as follows.First group (matched group) do not receive treatment.The 2nd group (matched group) accepted to carry the non-targeted restructuring minicell of plasmid pORF5-HSV1tk::Sh ble (being called M-HSVtk) at the 21st, 28 and 35 day.Mice was accepted GCV equally at the 25th, 26,32,33,39 and 40 day, namely continuous 2 days acceptance 2 dosage GCV.This group is designed to measure, and can non--targeting minicell be delivered to suicide gene tumor cell and affect tumor regression after the GCV treatment.Whether the 3rd group (matched group) is designed to be determined at when lacking GCV influential to tumor regression with the targeting restructuring minicell treatment of carrying plasmid pORF5-HSV1tk::Sh ble.Therefore, the 3rd group of mice accepted to carry the targeting restructuring minicell of plasmid pORF5-HSV1tk::Sh ble (being called TM-HSVtk) with the 2nd group of same natural law but do not accepted the GCV treatment.Whether bi-specific antibody was influential to tumor regression when the 4th group (matched group) was designed to be determined at shortage restructuring minicell.Therefore, these mices are accepted bi-specific antibody on the same day (namely the 21st, 28 and 35 day) that give recombinant target or non-targeted minicell.Then carry out the GCV treatment with the 2nd group of same natural law behind the Antybody therapy.Whether the 5th group (experimental group) is designed to measure the targeting restructuring minicell that carries plasmid pORF5-HSV1tk::Sh ble can effectively be delivered to plasmid the xenotransplantation tumor cell, and whether can observe tumor regression after treating mice with single dose GCV behind each minicell dosage.Therefore, accepting targeting restructuring minicell with the 3rd group of same natural law, then accepting the GCV treatment at the 25th, 33 and 39 day for the 5th group.The 6th group (experimental group) is identical with the 5th group but accept the continuously GCV of day 2 dosage as the 2nd and 4 group.
Be suspended in 10 in the 30 microlitre physiological saline solution with various
8Be administered to the mice of accepting various minicells in the individual small cell tumor.External gene target experiment demonstration in the MDA-MB-468 cell is sent the minicell of plasmid and is being expressed the HSVtk enzyme at least after 48 hours with the transfection of targeting restructuring minicell.Therefore, the 2nd, 4,5 and 6 group after minicell inoculation, gave GCV in 3 to 4 days so that the tumor xenotransplantation cell of transfection can effective expression HSVtk enzyme so that GCV is reacted.GCV gives with the heavy concentration intraperitoneal of 100 mg/kgs of Mus.
Fig. 5 shows the progress of gross tumor volume in the experiment process.The result shows that only targeting restructuring minicell (the 5th and 6 group) can successfully be delivered to the xenotransplantation tumor cell with HSV1tk gene code plasmid.The gross tumor volume size does not increase in these two groups, and keeps stable in whole experimentation.In contrast, gross tumor volume increases sharply in four matched groups (1-4 group).What is interesting is that the 2nd group of mice do not show the tumor regression sign equally, point out non--targeting restructuring minicell can not the transfection mankind mastopathy cell and can not obtain clinically significant result.Use the statistical data analysis of one way analysis of variance (One-way ANOVA) to show that experimental group (5 and 6) and matched group 1 to 4 compare highly significant (p=0.001).This result is the excess syndrome the earliest that by the complete restructuring minicell mediation that is derived from antibacterial gene target is delivered to non-phagocytic mammalian cells in the body.The endocytosis of the receptor-mediated minicell of its same proof realize highly effectively with gene delivery to the effect aspect these non-phagocytic mammalian cells (with the 2nd group with the 5th and 6 group relatively).
This experimental result shows that compositions of the present invention and method are used for the effectiveness of the mammalian cell that the minicell targeting is required in vivo.This class result proves the clinical practice that the targeting minicell is potential equally, especially aspect the exploitation cancer therapy.
Embodiment 6. carries and crosses effectively disappear tumor in the nude mice of the EGF receptor of expressing on the minicell targeting human breast cancer xenograft of suicide plasmid
Above-mentioned xenotransplantation research is implemented by (i.t.) injection minicell in the tumor.For assess in vivo by system send with the minicell targeting non--engulf (human cancer cell) cell surface receptor and reach the potential of the purpose that tumor stablize/disappears, designed another xenotransplantation research, wherein minicell is by intravenous injection.
Equally, structure and purification carry the restructuring minicell of plasmid pORF5-HSV1tk::Sh ble (HSV1tk).With the verified human EGFR of expressing of in mankind mastopathy cell MDA-MB-468, crossing of this class minicell targeting.It can contain the anti-human class EGFR of tool and the specific bi-specific antibody of anti-mouse typhus LPS and this BsAb is attached to the minicell surface by structure as described in Example 1 finishes.Subcutaneous between the scapula of nude mice (s.c.) sets up xenograft (every group of n=11), the experiment and the contrast minicell all shown in natural law (Fig. 6) in tail vein medium-sized vein, give.2nd, 4,6 and 7 groups shown in natural law accept equally GCV (i.p.).
Result's demonstration is only being used EGFR-targeting minicell
HSV1tkIn the mice for the treatment of the tumor of having set up had and stablize/disappear significantly.Every dosage 10
8Or 10
9These two kinds of minicell dosage tool same effect show that targeted approach is very efficient, and improve therapeutic index, so that carrier concn is not restriction factor.Use the statistical data analysis of one way analysis of variance to show that the result of experimental group (6 and 7) and matched group 1 to 5 relatively are highly significant (p=0.0001).Even these data show that minicell targeting technology is still very efficient aspect the tumor mass that minicell is led away from the site injection of tumor the time.These data show that equally system sends the toxicity that the targeting minicell can not cause to mice any manifest symptom.During whole research, not such as the toxicity of heating, drowsiness, poor appetite, weight saving or the manifest symptom such as dead.
Embodiment 7. carries on the minicell targeting human breast cancer xenograft of suicide plasmid low HER2/neu receptor of the expressing nude mice tumor that effectively disappears
The interior result of above-mentioned body points out can be with the expressed receptor of crossing on the minicell efficient targeting disease cell (for example cancer cell).Present embodiment shows the effect when minicell carrier targeting one is expressed very low cancer cell surface receptor.In traditional method, the low expressed receptor of targeting is that exploitation is based on the serious obstacle of the therapy of antibody, especially to treatment of cancer, because a lot of cancer cell can not be crossed expression target receptor.For example, the HER2/neu receptor was to express in being lower than 20% patient with breast cancer.
Equally, the xenotransplantation research design is minicell wherein
HSV1tkThe carrier targeting is known to the low HER2/neu receptor of expressing of MDA-MB-468 breast cancer cell.Except comprising another wherein intratumor injection HER2/neu-targeting minicell
HSV1tkOutside the experimental group (the 8th group), experimental group and matched group (Fig. 7) are identical with embodiment 6.Result (Fig. 7) is although showing that this HER2/neu receptor is low expresses, reach tumor stablize/disappear aspect the purpose experimental therapy just as embodiment 6 in minicell
HSV1tkThe EGF receptor situation that the carrier targeting is crossed expression is equally effective.Need identical targeting minicell for reaching this result
HSV1tkDosage number of times (3x).In this experiment, in case residual tumor began growth between the 53rd day and 81 days, give the HER2/neu targeting minicell of the 4th dosage
HSV1tk, in the 6th group and the 7th group, cause that gross tumor volume dwindles fast.Use the statistical data analysis of one way analysis of variance to show that experimental group (6,7 and 8) and matched group 1 to 5 compare highly significant (p=0.0001).
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Claims (5)
1. compositions, it comprises that (i) is derived from the minicell of antibacterial, it contains therapeutic nucleic acid molecule, reach (ii) bispecific part, it can be combined with described minicell surface texture and non-phagocytic mammalian cells surface receptor, described mammalian cell surface receptor can activated receptor the endocytosis of described minicell of mediation;
Wherein said minicell comprises the intact cell wall; Described therapeutic nucleic acids is comprised on the plasmid that is comprised of the Polynucleotide sequence.
2. the compositions of claim 1, wherein said minicell comprise the described plasmid of 11-60 copy.
3. the compositions of claim 1, wherein said minicell comprise the described plasmid that surpasses 60 copies.
4. claim 1 or 2 compositions, wherein said mammalian cell surface receptor overexpression is in described cell surface.
5. each compositions is in the purposes of preparation in the medicine among the claim 1-4, and described medicine is used for the treatment of disease or changes characteristic by being given cell, tissue or organ.
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- 2004-12-08 DE DE602004031870T patent/DE602004031870D1/en active Active
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Patent Citations (3)
Publication number | Priority date | Publication date | Assignee | Title |
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CN1278739A (en) * | 1997-09-15 | 2001-01-03 | 遗传免疫有限公司 | Method of delivering genes to antigen presenting cells of the skin |
WO2003033519A2 (en) * | 2001-10-15 | 2003-04-24 | Engeneic Gene Therapy Pty Limited | Intact minicells as vectors for dna transfer and gene therapy in vitro and in vivo |
US20030203481A1 (en) * | 2002-02-25 | 2003-10-30 | Surber Mark W. | Conjugated minicells |
Also Published As
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CN1913923B (en) | 2010-12-08 |
ES2362881T3 (en) | 2011-07-14 |
US9987377B2 (en) | 2018-06-05 |
US20180369416A1 (en) | 2018-12-27 |
PL1694361T3 (en) | 2011-08-31 |
US9169495B2 (en) | 2015-10-27 |
WO2005056749A3 (en) | 2005-10-13 |
AU2004297414B2 (en) | 2008-10-30 |
JP4332558B2 (en) | 2009-09-16 |
EP2295084A1 (en) | 2011-03-16 |
US20150343092A1 (en) | 2015-12-03 |
NZ547983A (en) | 2009-05-31 |
CN1913923A (en) | 2007-02-14 |
EP1694361A4 (en) | 2006-12-13 |
WO2005056749A2 (en) | 2005-06-23 |
CA2549840A1 (en) | 2005-06-23 |
HK1095090A1 (en) | 2007-04-27 |
EP1694361A2 (en) | 2006-08-30 |
DE602004031870D1 (en) | 2011-04-28 |
ATE501735T1 (en) | 2011-04-15 |
AU2004297414A1 (en) | 2005-06-23 |
PT1694361E (en) | 2011-06-27 |
US10583200B2 (en) | 2020-03-10 |
EP1694361B1 (en) | 2011-03-16 |
CA2549840C (en) | 2012-03-20 |
JP2007534310A (en) | 2007-11-29 |
CN101954095A (en) | 2011-01-26 |
AU2004297414C1 (en) | 2009-06-25 |
US20070237744A1 (en) | 2007-10-11 |
DK1694361T3 (en) | 2011-06-06 |
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